K of Dehm et al [6] suggested AR spliced variants (AR1/2/2b and AR1/2/3/2b) are largely responsible for the generation of the truncated receptors in CWR22Rv1. Work by Hu et al [7] and Guo et al [8], ML 281 web identified several additional spliced variants and found that AR3/AR-V7, but not AR1/2/2b or AR1/2/3/2b is the predominant species in CWR22Rv1. Guo et al, went on to develop antibodies against AR3 and conclusively identified the presence of the truncated receptor corresponding to AR3. While the direct demonstration of a cleaved product at the protein level is more challenging than the detection of spliced transcripts, none of the CAL-120 site studies have excluded the contributions of truncated receptor generated by proteolytic cleavage. Indeed, Hornberg et al [9] showed that there is a disparity between the amount of truncated receptor and the levelModeling Truncated AR in AD Backgroundof spliced variants. We therefore favor the hypothesis that truncated receptors can be generated through both proteolytic cleavage and alternative splicing. The schematic structure of the prototypic AR truncated variants in our reports as well as in other studies is shown in Figure 1A. Based on the protease cleavage model, the truncated AR would have a duplicated exon 3 and a C-terminal putative calpain cleavage site in the hinge region (Figure 1A (i)). The most abundant and well characterized splice variant is AR3/AR-V7 which has a similar structure except the last 16 C-terminal amino acids are derived from a cryptic exon (CE3) [7,8,10]. Another recent study also found a novel human AR splice variant (ARv567es) from prostate cancer xenografts with exons 5, 6, and 7 deleted, which is constitutively active in prostate cancer cell lines [11]. There are other splice variants similar to these prototypes, which are present less abundantly in prostate cancer cell line or tissues, and of which the protein products have yet to be identified [10,12,13]. These variants all lack the major part 1676428 of the ligand binding domain and their activities are ligand-independent. Although in FL-AR the hinge domain is required for nuclear localization [14], most reported splice variants are lacking the hinge region (and the nuclear localization signal encoded within it). However, as in the case of AR3/AR-V7, this deletion may be compensated for by a cryptic exon rich in lysine residues [12]. Most of the previous studies on truncated receptors have focused on their ability to transactivate androgen-responsive genes and to induce androgen-independent 24786787 growth [6?]. These studies were carried out primarily either in androgen-insensitive, AR negative cells, or in androgen-responsive cells with a high level of FL-AR, which preclude the analysis of isolated TC-AR in its natural androgen-responsive background. The presence of FL-AR apparently can affect the function of the spliced variants in a cell context dependent manner [10,15]. Furthermore, most of the biological studies utilize clones derived from transduction or transfection of cDNA carrying truncated receptors, which may have acquired properties different from the parental cells. As a potentially more attractive model, we present here the establishment of LN/TC-AR, a novel cell line derived from the androgen dependent LNCaP parental line in which expression of a Cterminally truncated AR (TC-AR) is regulated and titratable by doxycycline and automatically down modulates the expression of the endogenous FL-AR. As such, when uninduced, the main AR spe.K of Dehm et al [6] suggested AR spliced variants (AR1/2/2b and AR1/2/3/2b) are largely responsible for the generation of the truncated receptors in CWR22Rv1. Work by Hu et al [7] and Guo et al [8], identified several additional spliced variants and found that AR3/AR-V7, but not AR1/2/2b or AR1/2/3/2b is the predominant species in CWR22Rv1. Guo et al, went on to develop antibodies against AR3 and conclusively identified the presence of the truncated receptor corresponding to AR3. While the direct demonstration of a cleaved product at the protein level is more challenging than the detection of spliced transcripts, none of the studies have excluded the contributions of truncated receptor generated by proteolytic cleavage. Indeed, Hornberg et al [9] showed that there is a disparity between the amount of truncated receptor and the levelModeling Truncated AR in AD Backgroundof spliced variants. We therefore favor the hypothesis that truncated receptors can be generated through both proteolytic cleavage and alternative splicing. The schematic structure of the prototypic AR truncated variants in our reports as well as in other studies is shown in Figure 1A. Based on the protease cleavage model, the truncated AR would have a duplicated exon 3 and a C-terminal putative calpain cleavage site in the hinge region (Figure 1A (i)). The most abundant and well characterized splice variant is AR3/AR-V7 which has a similar structure except the last 16 C-terminal amino acids are derived from a cryptic exon (CE3) [7,8,10]. Another recent study also found a novel human AR splice variant (ARv567es) from prostate cancer xenografts with exons 5, 6, and 7 deleted, which is constitutively active in prostate cancer cell lines [11]. There are other splice variants similar to these prototypes, which are present less abundantly in prostate cancer cell line or tissues, and of which the protein products have yet to be identified [10,12,13]. These variants all lack the major part 1676428 of the ligand binding domain and their activities are ligand-independent. Although in FL-AR the hinge domain is required for nuclear localization [14], most reported splice variants are lacking the hinge region (and the nuclear localization signal encoded within it). However, as in the case of AR3/AR-V7, this deletion may be compensated for by a cryptic exon rich in lysine residues [12]. Most of the previous studies on truncated receptors have focused on their ability to transactivate androgen-responsive genes and to induce androgen-independent 24786787 growth [6?]. These studies were carried out primarily either in androgen-insensitive, AR negative cells, or in androgen-responsive cells with a high level of FL-AR, which preclude the analysis of isolated TC-AR in its natural androgen-responsive background. The presence of FL-AR apparently can affect the function of the spliced variants in a cell context dependent manner [10,15]. Furthermore, most of the biological studies utilize clones derived from transduction or transfection of cDNA carrying truncated receptors, which may have acquired properties different from the parental cells. As a potentially more attractive model, we present here the establishment of LN/TC-AR, a novel cell line derived from the androgen dependent LNCaP parental line in which expression of a Cterminally truncated AR (TC-AR) is regulated and titratable by doxycycline and automatically down modulates the expression of the endogenous FL-AR. As such, when uninduced, the main AR spe.